Exosome comprising photocleavable protein, and use thereof

ABSTRACT

The present disclosure relates to an exosome comprising a photocleavable protein and a use thereof, and the exosome according to the present disclosure contains a fusion protein comprising a blue fluorescent protein (TagBFP), a photocleavable protein (mMaple3), and an exosome-specific marker protein (CD9), and it has been found that when light of 405 nm is irradiated to the exosome, the photocleavable protein, mMaple3 is cleaved and thereby the blue fluorescent protein in the exosome can be delivered into a target cell. In addition, it has been found that Cre protein in the exosome can be delivered into an animal organ, when light of 405 nm is irradiated to an exosome containing Cre fusion protein (Cre-mMaple3-CD9). Therefore, the exosome containing the photocleavable protein according to the present disclosure is expected to be useful in the protein treatment field by safely and efficiently delivering various therapeutic proteins into cells.

CROSS REFERENCE TO RELATED APPLICATIONS

The present application is a National Phase of International Application No. PCT/KR2021/001634 filed on Feb. 8, 2021, which claims the priority benefit of Korean Patent Application Nos. 10-2020-0015696, filed on Feb. 10, 2020, and 10-2021-0015837, filed on Feb. 4, 2021, in the Korean Intellectual Property Office, the disclosures of which are incorporated herein by reference.

TECHNICAL FIELD

The present disclosure relates to an exosome comprising a photocleavable protein and a use thereof, and more specifically, relates to an exosome containing a fusion protein comprising a target protein and a photocleavable protein, mMaple3 and a use thereof.

The present application claims the priority based on Korean Patent Application No. 10-2020-0015696 filed on Feb. 10, 2020 and Korean Patent Application No. 10-2021-0015837 filed on Feb. 4, 2021, and the entire contents disclosed in the description and drawings of the corresponding applications are incorporated in the present application.

BACKGROUND ART

Most current protein therapies target cell membrane proteins. However, pathogenic factors of many diseases mainly exist inside the cell, and in order to target these pathogenic factors, a technology for delivering a therapeutic protein into the cell is required.

Accordingly, recently, a number of methods for introducing a target protein directly into a cell have been studied, and one of these, a technology of delivery of a therapeutic protein using a lipid nanoparticle has a problem in that the lipid nanoparticle is not effectively separated from the therapeutic protein, and a technology for delivery using a protein transduction domain (PTD) which plays a major role in the intracellular penetration process of viruses has a problem in that the protein transduction domain is degraded when exposed to body fluids such as blood or intestinal fluid.

Therefore, there is a need for a technology for effectively delivering a therapeutic protein to the inside of a cell in order to target pathogenic factors of a specific disease present inside the cell.

On the other hand, an exosome is a vesicle composed of a lipid-bilayer, and is a constituent of a substance secreted by a cell to the outside of the cell. In order to perform a functional role in mediating cell-cell communication and cellular immunity, the exosome is known to play a role of transporting (delivering) a protein, a bioactive lipid and RNA (miRNA) which are biomolecules in a cell. This exosome is also being studied as a biomarker for neurological disease such as Alzheimer, and the like, and is also used in development of a drug delivery system such as a nanocarrier of a specific drug due to high selective permeability enough to penetrate a blood-brain barrier (BBB) that separates cerebrospinal fluid and blood.

With respect to the technology for delivering a therapeutic protein, Korean Patent Publication No. 10-2018-0036134 discloses a method for preparation of an exosome comprising a super-repressor-Iκ protein using a light-specific binding protein, and a pharmaceutical composition for preventing and treating inflammatory disease containing the exosome prepared by the method for preparation as an active ingredient, and Japanese Patent Application Publication No. 2019-528674 discloses a method for mass production of an exosome comprising a cargo protein, a vector for preparing the exosome, an exosome comprising a cargo protein prepared by the method, and a method for loading a cargo protein on cytosol by using the exosome prepared thereby.

However, the above documents disclose a light-specific binding protein as a component of a fusion protein in an exosome, and this uses two light-specific binding proteins as CIBN-CRY2 system, so two constructs must be co-transfected when it is expressed in a cell, and therefore the efficiency is lowered, and 488 nm light must be continuously applied to the cell while exosomes are generated, so it may affect the cell, and loss of the amount of a transport protein contained in exosomes occurs. In addition, there are disadvantages in that when binding of CIBN and CRY2 is maintained in absence of light after exosome formation, the transport protein cannot move freely and may be bound to an exosome-specific protein, and the size of CRY2 to be fused to the transport protein is big as 65 kDa, so it may affect the intrinsic function of the transport protein, and in order to confirm whether it is expressed well in a cell, a fluorescent protein such as EGFP must be fused separately and used, and there is no way to confirm whether the binding of CRY2 and CIBN is fallen when no light is given.

Accordingly, the present inventors have attempted to overcome disadvantages of the conventionally known protein delivery technology using the CIBN-CRY2 system and develop a method for safely and effectively delivering a protein into a cell.

DISCLOSURE Technical Problem

The Sequence Listing created onSep. 14, 2022 with a file size of 11.00 KB, and filed herewith in ASCII text file format as the file entitled “Updated_Sequence.TXT,” is hereby incorporated by reference in its entirety.

The present inventors have found that when light is irradiated to an exosome containing a fusion protein where photocleavable protein mMaple3 is combined with a target protein to be delivered into a cell, the mMaple3 is cleaved to safely and efficiently release the target protein in the exosome into a target cell, thereby completing the present disclosure based on this.

Accordingly, an object of the present disclosure is to provide an exosome containing a fusion protein comprising a target protein, a photocleavable protein and an exosome-specific marker protein and a use thereof.

However, a technical problem to be achieved by the present disclosure is not limited to the aforementioned problems, and other problems not mentioned can be clearly understood by those skilled in the art to which the present disclosure pertains from the description below.

Technical Solution

In order to achieve the above objects, the present disclosure provides an exosome containing a fusion protein comprising a target protein and mMaple3.

In addition, the present disclosure provides a composition for delivery of a target protein into a cell, comprising the exosome as an active ingredient.

Moreover, the present disclosure provides a method for delivering a target protein into a cell in vitro, comprising irradiating light to an exosome containing a fusion protein comprising a target protein and mMaple3; and

treating the light-irradiated exosome to a target cell.

Furthermore, the present disclosure provides a screening method of a protein candidate drug for delivery into a cell, comprising

-   (a) irradiating light to an exosome containing a fusion protein     comprising a protein candidate drug and mMaple3; -   (b) treating the light-irradiated exosome to a target cell; and -   (c) confirming that the protein candidate drug is delivered into the     cell, when the mMaple3 exhibits fluorescence in the target cell.

As one embodiment of the present disclosure, the fusion protein may further comprise an exosome-specific marker protein.

In addition, the present disclosure provides a method for preparation of the fusion protein, comprising the following steps:

-   (S1) amplifying cDNA of a target protein and mMaple3, respectively; -   (S2) combining the amplified cDNA of the target protein and mMaple3     into one cDNA, to prepare cDNA encoding a fusion protein comprising     the target protein and mMaple3; and -   (S3) expressing the fusion protein by introducing cDNA encoding the     fusion protein into a vector and then transfecting it into a cell.

Furthermore, the present disclosure provides a method for preparation of the exosome, comprising the following steps:

-   (S1) amplifying cDNA of a target protein and mMaple3, respectively; -   (S2) combining the amplified cDNA of the target protein and mMaple3     into one cDNA, to prepare cDNA encoding a fusion protein comprising     the target protein and mMaple3; and -   (S3) transfecting cDNA encoding the fusion protein into an     exosome-producing cell, and separating and purifying an exosome from     a cell culture medium.

As one embodiment of the present disclosure, it may comprise combining the amplified cDNA of mMaple3 and cDNA of an exosome-specific marker protein into one cDNA, before combining the amplified cDNA of the target protein and mMaple3 into one cDNA in the (S2).

As another embodiment of the present disclosure, the separation of the exosome in the (S3) may use one method selected from the group consisting of TFF (tangential flow filtration), ultracentrifugation, size exclusion chromatography, and exosome isolation kit.

As other embodiment of the present disclosure, the mMaple3 may comprise the amino acid sequence of SEQ ID NO: 1.

As other embodiment of the present disclosure, the mMaple3 may be encoded by a gene comprising the nucleotide sequence of SEQ ID NO: 2.

As other embodiment of the present disclosure, the target protein may be a protein to be delivered into a cell.

As other embodiment of the present disclosure, the target protein may be a protein for treating disease or a protein for diagnosing disease.

As other embodiment of the present disclosure, the exosome-specific marker protein may be one or more selected from the group consisting of CD9, CD63, and CD81.

As other embodiment of the present disclosure, the mMaple3 in the exosome may be cleaved through the step of irradiating light to the exosome.

As other embodiment of the present disclosure, the light may have a wavelength of 401 nm to 480 nm.

In addition, the present disclosure provides a method for delivery into a cell of a target protein, comprising a method for administering a composition comprising an exosome containing a fusion protein comprising a target protein and mMaple3 into a subject.

Moreover, the present disclosure provides a use for delivering a target protein into a cell, of a composition comprising an exosome containing a fusion protein comprising a target protein and mMaple3.

Furthermore, the present disclosure provides a use of an exosome containing a fusion protein comprising a target protein and mMaple3, for production of a preparation for delivery into a cell of a target protein.

Effects

The exosome according to the present disclosure contains a fusion protein comprising a blue fluorescent protein (TagBFP), a photocleavable protein (mMaple3), and an exosome-specific marker protein (CD9), and it has been confirmed that when light of 405 nm is irradiated to the exosome, the photocleavable protein, mMaple3 is cleaved and thereby the blue fluorescent protein in the exosome can be delivered into a target cell. In addition, it has been confirmed that Cre protein in the exosome can be delivered into an animal organ, when light of 405 nm is irradiated to an exosome containing Cre fusion protein (Cre-mMaple3-CD9). Therefore, the exosome containing the photocleavable protein according to the present disclosure is expected to be usefully used in the protein treatment field by safely and efficiently delivering various therapeutic proteins into cells.

BRIEF DESCRIPTION OF THE DRAWINGS

The patent or application file contains at least one drawing executed in color. Copies of this patent or patent application publication with color drawing(s) will be provided by the Office upon request and payment of the necessary fee.

The patent or application file contains at least one drawing executed in color. Copies of this patent or patent application publication with color drawing(s) will be provided by the Office upon request and payment of the necessary fee.

FIG. 1 schematically shows the structure of the fusion protein in which the target protein (blue fluorescent protein), photocleavable protein and exosome-specific marker protein are combined according to one embodiment of the present disclosure and characteristics thereof.

FIG. 2 shows the process of preparation and the result of confirming expression in a cell of the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure.

FIG. 3 a briefly schematically shows the CIBN-CRY2 system.

FIG. 3 b briefly schematically shows the mMaple system according to one embodiment of the present disclosure.

FIG. 4 a is the result of confirming the cleavage effect by light irradiation of the fusion protein (TagBFP-mMaple3-CD9) in the HEK293T cell according to one embodiment of the present disclosure through a confocal microscope.

FIG. 4 b shows the intensity of fluorescence shown in FIG. 4 a above as a graph.

FIG. 4 c is the result of confirming the cleavage effect by light irradiation of the fusion protein (TagBFP-mMaple3-CD9) in the HEK293T cell according to one embodiment of the present disclosure by western blot.

FIG. 5 schematically shows the separation and purification process of the exosome according to one embodiment of the present disclosure.

FIG. 6 a is the result of measuring the size of the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure by NTA.

FIG. 6 b is the result of measuring the size of the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure by DLS.

FIG. 6 c is the result of measuring the concentration of the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure by microBCA.

FIG. 6 d is the result of measuring the zeta potential of the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure.

FIG. 6 e is the result of cryogenic electron microscopy (Cryo-TEM) image observation of the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure.

FIG. 6 f is the result of confirming the cleavage effect by light irradiation of the fusion protein (TagBFP-mMaple3-CD9) in the exosome according to one embodiment of the present disclosure by western blot.

FIG. 6 g is the result of confirming the cleavage effect by light irradiation of the fusion protein (TagBFP-mMaple3-CD9) in the exosome according to one embodiment of the present disclosure and whether the blue fluorescent protein is contained in the exosome by fluorescence intensity measurement.

FIG. 7 is the result of confirming whether the target protein is decomposed according to presence or absence of treatment of Triton X-100, proteinase (proteinase K), and light, to the exosome containing the fusion protein (TagBFP-mMaple3-CD9) according to one embodiment of the present disclosure.

FIGS. 8 a and 8 b are results of confirming the effect of delivery into a cell of the blue fluorescent protein in the exosome according to one embodiment of the present disclosure.

FIG. 9 is the result of confirming the effect of delivery in an animal organ of Cre protein in the exosome when the exosome contains the fusion protein (Cre-mMaple3-CD9) according to one embodiment of the present disclosure into an animal.

MODE FOR INVENTION

The present disclosure provides an exosome containing a fusion protein comprising a target protein and mMaple3.

In addition, the present disclosure provides a composition for delivery of a target protein into a cell, comprising the exosome as an active ingredient.

Furthermore, the present disclosure provides a method for preparation of the fusion protein comprising the following steps:

-   (S1) amplifying cDNA of a target protein and mMaple3, respectively; -   (S2) combining the amplified cDNA of the target protein and mMaple3     into one cDNA, to prepare cDNA encoding a fusion protein comprising     the target protein and mMaple3; and -   (S3) expressing the fusion protein by introducing cDNA encoding the     fusion protein into a vector and then transfecting it into a cell.

In addition, the present disclosure provides a method for preparation of the exosome comprising the following steps:

-   (S1) amplifying cDNA of a target protein and mMaple3, respectively; -   (S2) combining the amplified cDNA of the target protein and mMaple3     into one cDNA, to prepare cDNA encoding a fusion protein comprising     the target protein and mMaple3; and -   (S3) transfecting cDNA encoding the fusion protein into an     exosome-producing cell, and separating and purifying an exosome from     a cell culture medium.

In the present disclosure, it may comprise combining the amplified cDNA of mMaple3 and cDNA of an exosome-specific marker protein into one cDNA, before combining the amplified cDNA of the target protein and mMaple3 into one cDNA in the (S2).

In the present disclosure, the (S3) may be transfecting the cDNA encoding the fusion protein into an exosome-producing cell and replacing a cell culture medium with an FBS-free DMEM medium comprising penicillin/streptomycin and then collecting the medium, and separating and purifying an exosome from the collected medium.

In the present disclosure, the separation of the exosome in the (S3) may use one method selected from the group consisting of TFF (tangential flow filtration), ultracentrifugation, size exclusion chromatography, and exosome isolation kit, but not limited thereto.

In the present disclosure, “fusion protein” is a protein produced by fusion of two or more proteins, and may comprise a target protein and mMaple3, and may further comprise an exosome-specific marker protein. The target protein, mMaple3, and exosome-specific marker protein composing the fusion protein may be in a form combined into one, and for example, it may be in an order of the target protein-mMaple3-exosome-specific marker protein in order, and when tracking of the target protein is needed, it may be in an order of the exosome-specific marker protein-mMaple3-target protein, but there is no limitation on their binding order.

In the present disclosure, “target protein” is a protein present in an exosome in a form combined to a photocleavable protein, and means a protein to be delivered into a target cell or tissue. The target protein may be a protein for treating disease or a protein for diagnosing disease, and there is no limitation on type thereof. For example, a cancer inhibiting protein, p53 is delivered into a cancer cell as a target protein, and thereby, an effect of treating cancer may be exhibited, and an effect for treating Parkinson’s disease may be exhibited by delivering a normal parkin protein into a neuron for Parkinson’s disease caused by abnormal function due to mutation occurring in the parkin protein, and in the research of next-generation stem cell therapies, Oct4, Sox2, c-Myc, and Klf4 proteins as Yamanica factors which are proteins required in the most important process, a process of dedifferentiating a patient’s somatic cell into a stem cell are delivered into the patient’s somatic cell, and thereby, dedifferentiation into a stem cell is possible without a virus currently used for stem cell dedifferentiation. In addition, through delivery of a myodifferentiation inducing protein such as Myogenin and MyoD as a target protein, a therapeutic effect for degenerative muscle disease such as muscular dystrophy characterized by progressive muscle weakness, atrophy and muscle fiber necrosis, and the like may be shown, and through delivery of NRF2 and BDNF proteins known as having a protective effect of a cranial nerve in dementia, one of neurodegenerative diseases, a therapeutic effect for dementia may be exhibited, and through delivery of a brown fat inducing factor such as PGC1α, PPAR-γ which differentiate a white fat cell into a brown fat cell, a therapeutic effect for metabolic disease may be shown. In one embodiment of the present disclosure, using a blue fluorescent protein, TagBFP, delivery thereof into a cell has been confirmed, and using Cre protein, delivery thereof into an animal organ has been confirmed.

In the present disclosure, “delivery into a cell of a target protein” means transferring a target protein present in a form combined to a photocleavable protein in an exosome into the inside of a targeted cell from the exosome.

In the present disclosure, “mMaple3” is a photocleavable protein, and the “photocleavable protein” means a protein which is cleaved when exposed to light with a specific wavelength.

In the present disclosure, the mMaple3 may comprise the amino acid sequence of SEQ ID NO: 1, and may be encoded by a gene comprising the nucleotide sequence of SEQ ID NO: 2.

In the present disclosure, “exosome-specific marker protein” is a protein positioned at the exosome outer membrane, and for example, it may be one or more selected from the group consisting of CD9, CD63, and CD81, and according to one embodiment of the present disclosure may be CD9, but not limited thereto.

In the present disclosure, the CD9 may comprise the amino acid sequence of SEQ ID NO: 3, and may be encoded by a gene comprising the nucleotide sequence of SEQ ID NO: 4.

In the present disclosure, “exosome” is a membrane vesicle having a membrane structure composed of lipid bilayers secreted to the outside of a cell as collecting protein, DNA, RNA, and the like, for signaling between cells, and is present in body fluids in almost all eukaryotes. The diameter of the exosome may be 10 nm to 400 nm, 10 nm to 350 nm, 10 nm to 300 nm, 10 nm to 250 nm, 10 nm to 200 nm, 10 nm to 150 nm, 50 nm to 350 nm, 50 nm to 300 nm, 50 nm to 250 nm, 50 nm to 200 nm, 50 nm to 150 nm, 100 nm to 300 nm, 100 nm to 200 nm, or 100 nm to 150 nm, and when a multiple vesicle is fused with a cell membrane, it is released from a cell, or it is released from a cell membrane immediately.

The exosome may be prepared by using a method for extracting an exosome known in the art, and there is no limitation on the method for extracting.

In addition, the present disclosure provides a method for delivery into a cell of a target protein in vitro, comprising irradiating light to an exosome containing a fusion protein comprising a target protein and mMaple3; and

treating the light-irradiated exosome to a target cell.

In addition, the present disclosure provides a screening method of a protein drug for delivery into a cell, comprising (a) irradiating light to an exosome containing a fusion protein comprising a protein candidate drug and mMaple3;

-   (b) treating the light-irradiated exosome to a target cell; and -   (c) identifying the protein candidate drug as protein drug delivered     into the cell, if the mMaple3 exhibits fluorescence in the target     cell.

In the present disclosure, the mMaple3 in the exosome may be cleaved through the irradiating light into the exosome, and then, the light may have a wavelength of 401 nm to 480 nm, 401 nm to 470 nm, 401 nm to 460 nm, 401 nm to 450 nm, 401 nm to 440 nm, 401 nm to 430 nm, 401 nm to 420 nm, or 401 nm to 410 nm, and light of 400 nm or less is ultraviolet light (UV) and may damage it when treated to a cell or exosome, and light with a wavelength over 480 nm may also affect it when treated to a cell. In the present disclosure, there is no limitation on the wavelength of light as long as it is within a range of 401 nm to 480 nm, but according to one embodiment of the present disclosure, preferably, it may be 405 nm.

In the present disclosure, in the (c), the mMaple3 may exhibit green fluorescence when it is not cleaved, and may exhibit red fluorescence when cleaved.

In addition, the present disclosure provides a method for delivery into a cell of a target protein, comprising administering a composition comprising an exosome containing a fusion protein comprising a target protein and mMaple3 into a subject.

In the present disclosure, “subject” means a subject in need of the target protein, and more specifically, it means a primate which is a human or non-human, or a mammal such as a mouse, a dog, a cat, a horse and a cow.

In the present disclosure, “administration” means providing the prescribed composition of the present disclosure into a subject by any appropriate method.

Furthermore, the present disclosure provides a use for delivering a target protein into a cell, of the composition comprising an exosome containing a fusion protein comprising a target protein and mMaple3.

In addition, the present disclosure provides a use of the exosome containing a fusion protein comprising a target protein and mMaple3, for producing a preparation for delivering a target protein into a cell.

In one example of the present disclosure, a fusion protein (TagBFP-mMaple3-CD9) in which a blue fluorescent protein (TagBFP), a photocleavable protein (mMaple3) and an exosome-specific marker protein (CD9) were combined was prepared, and an advantage shown when the mMaple3 was used compared to other photocleavable protein types, and an advantage shown by the mMaple system compared to the CIBN-CRY2 system were confirmed (See Example 1).

In another example of the present disclosure, it was confirmed that the mMaple3 was cleaved by light of 405 nm, when the fusion protein (TagBFP-mMaple3-CD9) was overexpressed in the HEK293T cell, and then light of 405 nm was irradiated (See Example 2).

In other example of the present disclosure, it was confirmed that the mMaple3 was cleaved by light of 405 nm, when the exosome was separated and purified from the medium of the HEK293T cell in which the fusion protein (TagBFP-mMaple3-CD9) was overexpressed (See Example 3).

In other example of the present disclosure, as the result of confirming degradation of a target protein according to presence or absence of treatment of Triton X-100, proteinase (proteinase K) and light of 405 nm to an exosome containing the fusion protein (TagBFP-mMaple3-CD9), it was confirmed that the target protein was not degraded by proteinase and light of 405 nm did not affect the lipid bilayers of the exosome, unless artificially permeable to the lipid bilayers of the exosome by treating Triton X-100 (See Example 4).

In one experimental example of the present disclosure, it was confirmed that the blue fluorescent protein was delivered into a cell, when light of 405 nm was irradiated to the exosome containing the fusion protein (TagBFP-mMaple3-CD9) and this was treated to the HEK293T cell (See Experimental example 1).

In one experimental example of the present disclosure, it was confirmed that the Cre protein in the exosome was delivered into an organ of a mouse, when light of 405 nm was irradiated to the exosome containing the Cre fusion protein (Cre-mMaple3-CD9) and this was administered into a genetically modified mouse in which the red fluorescent protein (tdTomato) was expressed when the Cre protein was delivered (See Experimental example 2).

Hereinafter, in order to help understanding of the present disclosure, preferable examples and experimental examples are suggested. However, the following examples and experimental examples are provided only to understand the present disclosure more easily, but the content of the present disclosure is not limited by the following examples and experimental examples.

Example 1. Fusion Protein Preparation and Photocleavable Protein Characteristic Comparison 1-1. Fusion Protein Preparation

cDNA encoding the fusion protein (TagBFP-mMaple3-CD9) in which the blue fluorescent protein (TagBFP), photocleavable protein (mMaple3) and exosome-specific marker protein (CD9) were combined was prepared, and the structure of the fusion protein translated from the prepared cDNA and characteristics thereof were schematically shown in FIG. 1 , and the amino acid sequences of each of the TagBFP, mMaple3, and CD9 and the gene sequences encoding them were shown in Table 1 below.

TABLE 1 sequences SEQ ID Number mMaple 3 amino acid sequenc e MVSKGEETIMSVIKPDMKIKLRMEGNVNGHAFVIEGEGSGK PFEGIQTIDLEVKEGAPLPFAYDILTTAFHYGNRVFTKYPRKIPDYFKQSFPEGYSWERSMTYEDGGICNATNDITMEEDSFINKIHFKGTNFPPNGPVMQKRTVGWEVSTEKMYVRDGVLKGDV KMKLLLKGGSHYRCDFRTTYKVKQKAVKLPKAHFVDHRIEI LSHDKDYNKVKLYEHAVARNSTDSMDELYK 1 mMaple 3 DNA sequence ATGGTGAGCAAAGGCGAGGAGACAATCATGTCCGTGATC AAGCCCGACATGAAGATCAAACTGAGGATGGAGGGCAAC GTGAACGGCCACGCCTTCGTGATCGAGGGCGAAGGAAGC GGCAAGCCCTTCGAGGGCATCCAGACCATCGATCTGGAG GTCAAGGAGGGCGCTCCCCTCCCTTTCGCCTATGACATCCTGACCACCGCCTTCCACTACGGCAATAGGGTGTTCACCAAGTATCCCAGGAAGATCCCCGACTACTTCAAGCAGAGCTTCCCTGAGGGCTACAGCTGGGAGAGGAGCATGACATACGAGGACGGCGGCATCTGCAACGCCACCAACGACATCACAATGGAGGAGGACAGCTTCATCAACAAGATCCACTTCAAAGGCACAAACTTCCCCCCCAATGGCCCCGTGATGCAGAAGAGGACCGTGGGCTGGGAGGTGAGCACCGAGAAGATGTACGTGAGGGACGGCGTCCTGAAGGGCGACGTGAAGATGAAGCTCCTGCTCAAGGGCGGCAGCCACTACAGGTGCGACTTTAGGACCACCTATAAGGTGAAGCAGAAGGCTGTGAAGCTGCCCAAGGCCCACTTCGTCGACCATAGGATCGAGATCCTGTCCCACGACAAGGACTACAACAAGGTCAAGCTGTACGAGCACGCCGTCGCTAGGAACAGCACCGACAGCATGGACGAACTCTATAAG 2 CD9 amino acid sequence MPVKGGTKCIKYLLPGFNFIFWLAGIAVLAIGLWLRPDSQTKSIPEQETNNNNSSFYTGVYILIGAGALMMLVGFLGCCGAVQESQCMLGLFFGFLLVIFPAIEIAAAIWGYSHKDEVIKEVQEFYKDTYNKLKTKDEPQRETLKAIHYALNCCGLAGGVEQFISDICPKKDVLETFTYKSCPDAIKEVFDNKFHIIGAVGIGIAVVMIFGMIFSMILCCAIRRNREMV 3 CD9 DNA ATGCCGGTCAAAGGAGGCACCAAGTGCATCAAATACCTG CTGTTCGGATTTAACTTCATCTTCTGGCTTGCCGGGATTGC 4 sequenc e TGTCCTTGCCATTGGACTATGGCTCCGATTCGACTCTCAGACCAAGAGCATCTTCGAGCAAGAAACTAATAATAATAAT TCCAGCTTCTACACAGGAGTCTATATTCTGATCGGAGCCGGCGCCCTCATGATGCTGGTGGGCTTCCTGGGCTGCTGCGGGGCTGTGCAGGACTCCCAGTGCATGCTGGGACTGTTCTTCGGCTTCCTCTTGGTGATATTCGCCATTGAAATAGCTGCGGCCATCTGGGGATATTCCCACAAGGATGAGGTGATTAAGGAAGTCCAGGAGTTTTACAAGGACACCTACAACAAGCTGAAAACCAAGGATGAGCCCCAGCGGGAAACGCTGAAAGCCATCCACTATGCGTTGAACTGCTGTGGTTTGGCTGGGGGCGTGGAACAGTTTATCTCAGACATCTGCCCCAAGAAGGACGTACTCGAAACCTTCACCGTGAAGTCCTGTCCTGATGCCATCAAAGAGGTCTTCGACAATAAATTCCACATCATCGGCGCAGTGGGCATCGGCATTGCCGTGGTCATGATATTTGGCATGATCTTCAGTATGATCTTGTGCTGTGCTATCCGCAGGAACCGCGAGATGGTC TagBFP amino acid sequenc e MSELIKENMHMKLYMEGTVDNHHFKCTSEGEGKPYEGTQTMRIKVVEGGPLPFAFDILATSFLYGSKTFINHTOGIPDFFKQSFPEGPTWERVTTYEDGGVLTATQDTSLQDGCLIYNVKIRGVNFTSNGPVMQKKTLGWEAFTETLYPADGGLEGRNDMALKLVGGSHLLANIKTTYRSKKPAKNLKMPGVYYVDYRLERIKEANNETYVEQHEVAVARYCDLPSKLGHKLN 5 TagBFP DNA sequenc e ATGAGCGAGCTGATTAAGGAGAACATGCACATGAAGCTGTACATGGAGGGCACCGTGGACAACCATCACTTCAAGTGCACATCCGAGGGCGAAGGCAAGCCCTACGAGGGCACCCAGACCATGAGAATCAAGGTCGGTCGAGGGCGGCCCTCTCCCTTCGCCTTCGACATCCTGGCTACTAGCTTCCTCTACGGCAGCAAGACCTTCATCAACCACACCCAGGGCATCCCCGACTTCTTCAAGCAGTCCTTCCCTGAGGGCTTCACATGGGAGAGAGTCACCACATACGAAGACGGGGGCGTGCTGACCGCTACCCAGGACACCAGCCTCCAGGACGGCTGCCTCATCTACAACGTCAAGATCAGAGGGGTGAACTTCACATCCAACGGCCCTGTGATGCAGAAGAAAACACTCGGCTGGGAGGCCTTCACCGAGACGCTGTACCCCGCTGACGGCGGCCTGGAAGGCAGAAACGACATGGCCCTGAAGCTCGTGGGCGGGAGCCATCTGATC GCAAACATCAAGACCACATATAGATCCAAGAAACCCGCTAAGAACCTCAAGATGCCTGGCGTCTACTATGTGGACTACAGACTGGAAAGAATCAAGGAGGCCAACAACGAGACCTACGTCGAGCAGCACGAGGTGGCAGTGGCCAGATACTGCGACCTCCCTAGCAAACTGGGGCACAAGCTTAAT 6

Specifically, at first, cDNA encoding TagBFP, mMaple3 and CD9 was prepared and amplified by PCR, respectively, and cDNA of the amplified mMaple3 and CD9 was combined into one cDNA (mMaple3-CD9) by PCR. Then, mMaple3-CD9 cDNA and TagBFP cDNA were combined into one cDNA (TagBFP-mMaple3-CD9) by PCR to produce cDNA encoding a fusion protein. The primers used in the present disclosure were shown in Table 2 below.

TABLE 2 DNA fragmentfor cloning Primer sequence SEQ ID Number TagBFP-Linker F: TATGCTGAATTCGCCACCATGAGCGAG 7 R: GGAAGCTTGAGCTCGAGATCTGAGTCCGGAATTAAGCTTGTGCCCCAGTTTG 8 Linker-mMaple3-Linker F: TCTCGAGCTCAAGCTTCCGTGAGCAAAGGCGAGGAG 9 R: ACCTCCGCCTGAACCGCCACCTCCCGACTTATAGAGTTCGTCCATGCTGTC 10 Linker-CD9 F: GGCGGTTCAGGCGGAGGTGGCTCTGGCGGTGGCGGATCGCCGGTCAAAGGAGGCAC 11 R: CCCTCTAGTCTAGAGACCATCTCGCGGTTCC 12

After that, cDNA encoding a fusion protein was cloned by using EcoR1 and Xbal restriction enzymes into pCMV14 vector so that the fusion protein was expressed in Mammalia cell. When the pCMV14-TagBFP-mMaple3-CD9 was transfected into the HEK293T cell by using PEI (polyethylenimine), as shown in FIG. 2 , expression of the fusion protein was confirmed.

1-2. Comparison of Characteristics According to Photocleavable Protein Types

By comparing characteristics of various kinds of photocleavable proteins (PAFP) such as Dendra2, mEos2, tdEos, mKikGR, and Kaede, and the like, and mMaple3 by referring to conventional documents (S. Wang, et al, Proc. Natl. Acad. Sci. U.S.A. 111, 8452-8457 (2014)), an advantage shown by the mMaple3 when compared to other photocleavable proteins was confirmed.

As a result, as shown in Table 3 below, it was confirmed that many photocleavable proteins generally had strong tendency to form oligomers in oligomerization tendency and cohesion, whereas mMaple3 had strong tendency to maintain monomers and weak cohesion.

Regarding the result of Switch λ showing a wavelength of light for cleavage, it was confirmed that KikGR and Kaede required light of 400 nm or less to be cleaved, and 400 nm or less is UV (ultraviolet light) and may damage it when treated to a cell or exosome, whereas in case of irradiating light of 400 nm or more, it was safer when it was cleaved after expressing in a cell or it was cleaved by adding to the exosome, and the mMaple3 was cleaved with light of 400 nm or more.

Among the photocleavable proteins expressed in a cell, there may be photocleavable proteins that are not fully folded until fluorescence is measured, and among the photocleavable proteins that have been fully folded, only some of them are cleaved by light to show fluorescence, and it could be confirmed that the efficiency of being cleaved and showing fluorescence was superior to that of other photocleavable protein as the mMaple3 had a high level of No. of localizations per cell showing the number of PAFP (photoactivatable fluorescent protein) detected by fluorescence per cell/ the expression level of actual PAFP.

In addition, while most photocleavable proteins have acid sensitivity, there was no reported acid sensitivity in case of mMaple3.

TABLE 3 PAFP Oligomerization Clustering Switchλ (mm) No. of localizations per cell Acid Sensitivity Dendra2 Monomer - 405, 480 1,810 High mEos2 Weak dimes + 405 1,290 Moderate tdEos Tetramer - 405 1,800 NA mKikGR Monomer + 390 3,800 High Kaede Tetramer + 380 NA Moderate mMaple3 Monomer - 405 12,300 NA

1-3. Comparison of CIBN-CRY2 System and mMaple System

The CIBN-CRY2 system shown in FIG. 3 a uses two light-specific binding proteins, so two constructs should be always used, and in this case, as two constructs should be co-transfected, the efficiency is lowered. For example, when the transfection efficiency is 80%, the probability that all the two constructs are transfected into one cell becomes 64%. On the other hand, the mMaple system shown in FIG. 3 b uses one construct, so it is possible to express it in a cell with better efficiency.

In addition, the CIBN-CRY2 system has disadvantages in that it may affect a cell as light of 488 nm should be continuously applied into the cell during producing an exosome, and loss of the amount of the transport protein contained in the exosome is caused as the binding efficiency of CIBN and CRY2 by light cannot be 100%, but the mMaple system is safe as the transport protein is fused to a photocleavable protein and an exosome-specific marker at the beginning and therefore there is no transport protein loss when a cell forms an exosome, and light is not required to be applied directly to the cell.

Furthermore, in the CIBN-CRY2 system, the case in that the binding of CIBN and CRY2 is not maintained under the condition without light after forming an exosome may occur and in this case, the transport protein cannot move freely and may be bound to the exosome-specific protein, whereas the mMaple system cleaves the photocleavable protein by applying light to the exosome after forming an exosome, and then, the efficiency to be cleaved is very high, and when the cleavage efficiency is high, it means that a lot of transport proteins the can move freely are generated in the exosome.

Moreover, the CIBN-CRY2 system has disadvantages in that it cannot affect the intrinsic function of the transport protein as the size of CRY2 is big as 65 kDa, and a fluorescent protein such as EGFP should be fused and used separately to confirm whether it is expressed well in a cell, and there is no way to confirm whether the binding of CRY2 and CIBN is broken when light is not given, while the mMaple system has very low possibility to affect the intrinsic function of the transport protein as the size of the photocleavable protein fragment attached to the transported protein after being cleaved is just 10 kDa, and whether it is expressed properly in a cell can be confirmed by green fluorescence as the photocleavable protein itself is a fluorescent protein, and whether the photocleavable protein is delivered well can be confirmed by red fluorescence after treating light to the exosome.

As above, when the photocleavable protein mMaple3 according to the present disclosure is comprised in the fusion protein, compared to the case in that other type of photocleavable protein and a light-specific binding protein of the CIBN-CRY2 system are comprised, the advantage as in Examples 1-2 and 1-3 above are shown, and accordingly, an effect of protein delivery into a cell was confirmed by an experiment using a fusion protein comprising the photocleavable protein mMaple3 of the present disclosure.

Example 2. Confirmation of Delivery of Fusion Protein

24 hours after seeding the HEK293T cell, the TagBFP-mMaple3-CD9 cDNA was transfected using PEI by the method of Example 1-1 above to overexpress it into the HEK293T cell, and then an effect of cleavage by light was confirmed by a confocal microscope and western blot in the HEK293T cell by irradiating light of 405 nm.

The experimental result of confocal microscope observation confirmed the expression of the fusion protein using a confocal microscope (LSM700), 24 hours after transfection by blue fluorescence (TagBFP) and green fluorescence (mMaple3) in FIG. 4 a , and confirmed the delivery of the fusion protein by the reduced intensity of green fluorescence (mMaple3 before cleaved) and the increased intensity of red fluorescence (mMaple3 after cleaved), and the intensity of the fluorescence was measured and shown in FIG. 4 b .

As a result, as shown in FIGS. 4 a and 4 b , considering that green fluorescence of the mMaple3 itself was shown before irradiating light of 405 nm and red fluorescence was shown after irradiating light of 405 nm, it could be confirmed that the mMaple3 protein was cleaved, and it was confirmed that the longer the 405 nm light was irradiated, the more the photocleavable protein (mMaple3) was cleaved, so the green fluorescence was decreased and red fluorescence was increased.

In addition, light of 405 nm was irradiated into a cell for 5 minutes, 24 hours after transfection using western blot and the protein was extracted using T-per buffer, and the extracted protein was separated by electrophoresis and then the expression of the fusion protein and cleavage of the fusion protein by light of 405 nm were confirmed, and as a result, as shown in FIG. 4 c , by observing that after irradiating light of 405 nm, the amount of the fusion protein not cleaved was reduced over time, whereas the amount of the cleaved fusion protein section was increased, the effect of cleavage of the mMaple3 protein was confirmed in the HEK293T cell.

Example 3. Exosome Separation and Purification

From the medium of the HEK293T cell overexpressing the fusion protein in Example 2 above, the exosome was separated and purified by Tangential Fluid Filtration system.

Specifically, 24 hours after seeding the HEK293T cell, the TagBFP-mMaple3-CD9 cDNA was transfected by using PEI, and 24 hours after transfection, the cell culture medium was replaced with FBS-free DMEM (1% PS(penicillin/streptomycin)) medium. 24 hours after replacing the medium, the medium was collected primarily, and the FBS-free DMEM (1% PS) medium was added again, and after 24 hours, the medium was secondarily collected. The exosome was separated and purified from the medium collected primarily and secondarily by TFF (tangential flow filtration) method. The process of the separation and purification of the exosome was schematically shown in FIG. 5 .

After separating and purifying the exosome by the method, the concentration and size of the exosome containing the fusion protein were measured by NTA (Nanoparticle Tracking Assay), DLS (Dynamic Light Scattering) and microBCA (Bicinchoninic Acid Assay).

As the result of NTA measurement, as shown in FIG. 6 a , the average diameter of the exosome was shown as 132 nm, and as the result of DLS measurement, as shown in FIG. 6 b , the average diameter of the exosome was confirmed as 117.7±10.28 nm, and as the result of microBCA measurement, as shown in FIG. 6 c , the concentration of the protein of the exosome containing the fusion protein was shown as 1487 mg/mL, and it was confirmed that the amount of the protein contained in one exosome was 39.13 ng.

Furthermore, as the result of measuring a zeta potential of the exosome, as shown in FIG. 6 d , it was confirmed as -19.3±0.8 mV on the average, and cryogenic electron microscopy (Cryo-TEM) image observation data of the exosome were shown in FIG. 6 e (scale bar: 100 nm)

In addition, as the result of confirming the effect of cleavage of the fusion protein by light of 405 nm in the exosome by western blot, as shown in FIG. 6 f , by observing that the amount of the fusion protein not cleaved was reduced over time after irradiating light of 405 nm, whereas the amount of the cleaved fusion protein section was increased, the effect of cleavage of the mMaple3 protein was confirmed in the exosome.

As the result of measuring the intensity of blue fluorescence, green fluorescence and red fluorescence by BioTek microplate reader machine in order to confirm the effect of cleavage of the fusion protein by light of 405 nm and whether the blue fluorescent protein was contained in the exosome once more, as shown in FIG. 6 g , it was confirmed that the intensity of blue fluorescence had no difference before and after irradiating light of 405 nm, and it was observed that the intensity of green fluorescence was greatly reduced after irradiating light of 405 nm, whereas the intensity of red fluorescence was increased, and thereby, the effect of cleavage of the fusion protein in the exosome and whether the blue fluorescent protein was contained in the exosome were confirmed.

Example 4. Confirmation of Position of Target Protein in Exosome

In order to confirm the position of the target protein (TagBFP) in the exosome (+mMaple3 exosomes) containing the fusion protein (TagBFP-mMaple3-CD9), separated in Example 3 above, protease digestion assay was performed.

Specifically, degradation of the target protein according to treatment of Triton X-100 and proteinase (proteinase k) which enable permeation of lipid bilayers of the exosome was confirmed.

As a result, as shown in FIG. 7 , it could be found that unless the lipid bilayers of the exosome was artificially permeated by using Triton X-100, the protein (ALIX) present inside the exosome including the target protein (TagBFP) was not degraded and was well protected from the proteinase (proteinase k). On the other hand, it was confirmed that the protein (LAMP2) having a domain outside the exosome was degraded by the proteinase regardless of whether Triton X-100 was treated. In addition, it was confirmed that light of 405 nm did not affect the lipid bilayers of this exosome.

Experimental Example 1. Confirmation of Protein in Exosome Into Cell

To the exosome containing the fusion protein (TagBFP-mMaple3-CD9), separated in Example 3 above (+mMaple3 exosomes), and the exosome not containing a specific protein separated and purified from the HEK293T cell culture solution (+Negative exosomes) as a control group, light of 405 nm was treated and they were treated to the HEK293T cell.

Specifically, in 24 hours after seeding the HEK293T cell, the exosome containing the TagBFP-mMaple3-CD9 fusion protein was treated at a concentration of 5 x 10⁹ particles/mL, and in 24 hours after treating the exosome, the HEK293T cell was fixed with 4% paraformaldehyde and then delivery of the blue fluorescent protein was confirmed with cytation 5 cell imaging machine.

As a result, as shown in FIG. 8 a , it was observed that blue fluorescence (TagBFP) was shown in the cell when the exosome containing mMaple3 was treated, and it was confirmed that green fluorescence (FL mMaple3) was reduced and red fluorescence (CL mMaple3) was increased as light was treated to the exosome.

In addition, as the result of confirming delivery of the blue fluorescent protein in the cell after treating the exosome to the HeLa cell by the same method, as shown in FIG. 8 b , it was confirmed that blue fluorescence was also shown in the HeLa cell, and it was confirmed that green fluorescence was reduced and red fluorescence was increased when light was treated to the exosome.

From this, it could be confirmed that mMaple3 was cleaved by treatment of 405 nm light in the exosome containing TagBFP-mMaple3-CD9, and thereby, the blue fluorescent protein (TagBFP) was delivered into a cell.

Experimental Example 2. Confirmation of Delivery of Protein In Exosome into Animal Organ

Light of 405 nm was treated to the exosome containing the Cre fusion protein (Cre-mMaple3-CD9), separated by the method as Example 3 above, and when the Cre protein was delivered, it was administered into a genetically modified mouse in which the red fluorescent protein (tdTomato) was expressed.

Specifically, the exosome in which phosphate buffer saline (PBS) or light was treated into the genetically modified mouse (Cre:MAPLEX) 500 µg was administered into a tail vein, and then after 1, 6 and 24 hours, the intensity of red fluorescence was measured with IVIS small animal imaging machine.

As a result, as shown in FIG. 9 , it was confirmed that the intensity of red fluorescence was increased in the liver of the mouse in which the light-treated exosome was administered as shown in FIG. 9 . From this, it could be confirmed that mMaple3 was cleaved by treatment of 405 nm light in the exosome containing Cre-mMaple3-CD9, and thereby, the Cre protein was effectively delivered into an organ.[150] The description of the present disclosure described above is for illustration, and those skilled in the art to which the present disclosure pertains can understand that it can be easily modified into other specific forms without changing the technical spirit or essential features of the present disclosure. Therefore, it should be understood that the examples described above are illustrative and not restrictive in all respects.

INDUSTRIAL APPLICABILITY

The exosome containing a photocleavable protein according to the present disclosure is expected to be usefully used in the protein treatment field by safely and efficiently delivering various therapeutic proteins into cells. 

1. An exosome comprising a fusion protein which comprises a target protein and mMaple3.
 2. The exosome according to claim 1, wherein the mMaple3 comprises the amino acids of SEQ ID NO:
 1. 3. The exosome according to claim 1, wherein the mMaple3 is encoded by a gene comprising the nucleotides of SEQ ID NO:
 2. 4. The exosome according to claim 1, wherein the fusion protein further comprises an exosome-specific marker.
 5. The exosome according to claim 1, wherein the target protein is to be delivered into a cell.
 6. The exosome according to claim 5, wherein the target protein is for treating a disease or for diagnosing a disease.
 7. The exosome according to claim 4, wherein the exosome-specific marker is one or more selected from the group consisting of CD9, CD63 and CD81.
 8. A composition for delivery of a target protein into a cell, comprising the exosome according to claim 1 as an active ingredient.
 9. The composition according to claim 8, wherein the target protein is to be delivered into a cell.
 10. The composition according to claim 9, wherein the target protein is for treating a disease or for diagnosing a disease. 11-21. (canceled)
 22. A method of delivering a target protein into a cell, comprising: administering a composition comprising an exosome into a subject in need thereof, wherein the exosome comprises a fusion protein comprising a target protein and mMaple3. 23-24. (canceled) 